Methods for obtaining nucleotide sequences coding for polypeptides specifically active for larvae of S. littoralis

ABSTRACT

This invention relates to a method for the cloning a polypeptide having larvicidal activity. In particular, the invention relates to vectors, bacterial strains and methods for the cloning and expression of the N-terminal region of a polypeptide toxic against the larvae of Lepidoptera of the Noctuidae family, preferably against  S.littoralis.

This is a continuation of application Ser. No. 08/461,750, now U.S. Pat. No. 6,110,734, filed Jun. 5, 1995, which is a con of Ser. No. 08/251,622, filed May 31, 1994, now abandoned, which is a con of Ser. No. 08/094,382, filed Jul. 21, 1993, now abandoned, which is a con of Ser. No. 07/458,754 filed Dec. 11, 1989, now abandoned, which is a 371 of PCT/FR88/00292 filed Jun. 9, 1988.

The subject of the invention is nucleotide sequences coding for polypeptides endowed with a larvicidal activity towards Lepidoptera.

It relates more particularly to agents, in particular nucleotide sequences, polypeptides or even vectors, or bacterial strains modified by these sequences and expressing polypeptides making it possible to prepare larvicidal compositions active against Lepidoptera, preferably against Spodoptera littoralis (hereafter S.littoralis) or Mamestra brassicae (hereafter designated by M.brassicae) or capable of transforming the plants to be treated in conferring on them this type of activity.

BACKGROUND OF THE INVENTION

It is known that most of the isolates of B.thuringiensis show a toxic activity with regard to larvae of more than a hundred species of Lepidoptera.

This activity results from the capacity of the strains of B.thuringiensis to synthesize, at the moment of sporulation, crystalline inclusions of protein nature, or δ-endotoxins, under the control of one or several types of gene.

It has been shown that the activity of these polypeptides is contained in the NH₂-terminal half or N-terminus of the protein.

The studies carried out have shown the high specificity of the δ-endotoxins towards larvae of a given species.

On account of this high specificity, many species of Lepidoptera, in particular of the family of the Noctuidae, react only weakly to commercial preparations of available B.thuringiensis.

It is so in particular for the species S.littoralis, a poly-phagous insect which constitutes the principal parasite of cotton and other industrially important crops. Among these crops, mention should be made of maize, the castor oil plant, tobacco, the groundnut, fodder plants, such as clover or alfalfa, or also market garden produce such as the cabbage or the tomato.

Hence, one can imagine the interest of disposing of agents targeting specifically and effectively the family of the Noctuidae and in particular S.littoralis or M.brassicae.

The genes for δ-endotoxins hitherto identified do not code for a polypeptide preferentially active with regard to S.littoralis.

SUMMARY OF THE INVENTION

The search by the inventors for a sequence of nucleotides coding for a polypeptide preferably active against the Noctuidae, more especially against S.littoralis, has led them to study the natural isolates of two strains of B.thuringiensis, the larvicidal activity of which on S.littoralis appears to be higher than that of the industrial preparations made starting from other strains of B.thuringiensis.

The species in question are aizawai 7-29 and entomocidus 6-01.

The study of these isolates has made it possible to demonstrate the existence of several genes for δ-endotoxins of different structures and different specificities, of which two genes preferentially active against P.brassicae but not very active against the Noctuida of cotton and a gene inactive against P.brassicae and S.littoralis.

By studying the total DNA of these isolates and by carrying out appropriate hybridizations, followed by the cloning of the fragments identified by hybridization, the inventors have observed that it is possible to isolate nucleotide sequences implicated in genes for δ-endotoxins coding for polypeptides active, preferably, against S.littoralis.

Thus, the aim of the invention is to provide nucleotide sequences capable of coding for at least the NH₂-terminal part of a δ-endotoxin toxic against the Noctuidae and preferably against S.littoralis or M.brassicae.

It also has the aim of providing a polypeptide toxic with regard to the Noctuidae.

Furthermore, the invention relates to a procedure for obtaining such a sequence and a polypeptide showing the desired activity as well as the intermediate agents such as vectors and bacterial strains which can be utilized for obtaining the polypeptide.

In addition, the invention relates to the uses of these sequences and polypeptides for the development of larvicidal compositions with regard to the Noctuidae, in particular S.littoralis and for the transformation of the plants likely to be infected by these larvae.

The invention relates to a sequence of nucleotides coding for at least a part of the N-terminal region of a polypeptide toxic specifically against the larvae of Lepidoptera of the Noctuidae family, and preferably against S.littoralis, characterized by its capacity of hybridization with a gene capable of expressing a polypeptide toxic towards larvae of S.littoralis.

According to another aspect of the invention, the nucleotide sequence is characterized in that it is carried by a sequence of nucleotides of about 3 kb such as obtained by in vitro genetic recombination of sequences of nucleotides of B.thuringiensis capable of hybridizing with probes 1, 2 and 3 of pHTA2 shown in FIG. 2. The fragment of 3 kb corresponds more particularly to the restriction fragment HindIII-PstI.

The sequences of nucleotides of the invention are, in addition, characterized in that they contain sites in the following order: HindIII-HincII-BglII-KpnI-HindIII-PstI.

In a preferred manner, these sequences of nucleotides are obtained by in vitro genetic recombination of DNA sequences derived from at least one strain of B.thuringiensis. In a variant of the embodiment of the invention, two different strains of B.thuringiensis are utilized.

Strains of B.thuringiensis particularly suited for obtaining these sequences of nucleotides are the strains corresponding to aizawai 7-29 and entomocidus 6-01, deposited on Apr. 21, 1987 under the No. I-661 and No. I-660, respectively, with the National Collection of Cultures of Microorganisms (N.C.C.M.) in Paris.

In an advantageous manner, the sequences of nucleotides of the invention code, for a polypeptide capable of forming an immunological complex with antibodies directed against polypeptides showing the larvicidal activity with regard to S.littoralis.

DETAILED DESCRIPTION OF THE INVENTION

A sequence of nucleotides according to the invention is characterized in that it has the capacity to hybridize with a probe formed from the sequence (I) showing the following chain arrangement (nucleotides 52-990 of SEQ ID NO:1):

     52 GTC  TAC  TTG  ACA  GGG  GTA  GGA  ACA  TAA  TCG  GTC  AAT  TTT  AAA                                    112 TAT  GGG  GCA  TAT  ATT  GAT  ATT  TTA  TAA  AAT  TTG  TTA  CGT  TTT                                                                  172 TTG  TAT  TTT  TTC  ATA  AGA  TGT  GTC  ATA  TGT  ATT  AAA  TCG  TGG TAA  TGA  AAA  ACA  GTA  TCA  AAC  TAT  CAG  AAC  TTT  GGT  AGT  TTA                          232 ATA  AAA  AAA  CGG  AGG  TAT  TTT  ATG  GAG  GAA  AAT  AAT  CAA  AAT                                                        292 CAA  TGC  ATA  CCT  TAC  AAT  TGT  TTA  AGT  AAT  CCT  GAA  GAA  GTA CTT  TTG  GAT  GGA  GAA  CGG  ATA  TCA  ACT  GGT  AAT  TCA  TCA  ATT                352 GAT  ATT  TCT  CTG  TCA  CTT  GTT  CAG  TTT  CTG  GTA  TCT  AAC  TTT                                              412 GTA  CCA  GGG  GGA  GGA  TTT  TTA  GTT  GGA  TTA  ATA  GAT  TTT  GTA TGG  GGA  ATA  GTT  GGC  CCT  TCT  CAA  TGG  GAT  GCA  TTT  CTA  GTA      472 CAA  ATT  GAA  CAA  TTA  ATT  AAT  GAA  AGA  ATA  GCT  GAA  TTT  GCT                                    532 AGG  AAT  GCT  GCT  ATT  GCT  AAT  TTA  GAA  GGA  TTA  GGA  AAC  AAT                                                                  592 TTC  AAT  ATA  TAT  GTG  GAA  GCA  TTT  AAA  GAA  TGG  GAA  GAA  GAT CCT  AAT  AAT  CCA  GAA  ACC  AGG  ACC  AGA  GTA  ATT  GAT  CGC  TTT                          652 CGT  ATA  CTT  GAT  GGG  CTA  CTT  GAA  AGG  GAC  ATT  CCT  TCG  TTT                                                        712 CGA  ATT  TCT  GGA  TTT  GAA  GTA  CCC  CTT  TTA  TCC  GTT  TAT  GCT CAA  GCG  GCC  AAT  CTG  CAT  CTA  GCT  ATA  TTA  AGA  GAT  TCT  GTA                772 ATT  TTT  GGA  GAA  AGA  TGG  GGA  TTG  ACA  ACG  ATA  AAT  GTC  AAT                                              832 GAA  AAC  TAT  AAT  AGA  CTA  ATT  AGG  CAT  ATT  GAT  GAA  TAT  GCT GAT  CAC  TGT  GCA  AAT  ACG  TAT  AAT  CGG  GGA  TTA  AAT  AAT  TTA      892 CCG  AAA  TCT  ACG  TAT  CAA  GAT  TGG  ATA  ACA  TAT  AAT  CGA  TTA                                    952 CGG  AGA  GAC  TTA  ACA  TTG  ACT  GTA  TTA  GAT  ATC  GCC  GCT  TTC TTT  CCA  AAC  TAT  GAC

Sequences of nucleotides coding for at least a part of the N-terminal region of a polypeptide toxic specifically towards larvae of Lepidoptera of the Noctuidae family, and preferably towards S.littoralis, are characterized in that they contain the chain arrangement (I) defined above.

In an advantageous manner, the sequence of nucleotides characterized by the chain arrangement defined above codes for a part of a polypeptide having a higher larvicidal activity towards S.littoralis than that of the polypeptides encoded by natural isolates presently known for their effects against S.littoralis.

The study of this sequence of nucleotides shows that it is characterized by an initiation codon ATG situated at position 241 starting from which an open reading frame of 750 nucleotides has been identified.

This sequence is also characterized by a GGAGG attachment site for ribosomes at positions 230 to 234.

According to another feature, the sequence of nucleotides of the invention is characterized in that it contains, upstream from the ATG codon, a sequence going from the nucleotide at position 137 to the nucleotide at position 177, strongly homologous with the region found by Wong et al. (1983) and described in (16) upstream from the gene for the crystal of the strain kurstaki HD1 Dipel (BTK) and for which the authors have shown that it contains three promoters BtI, BtII and Ec which are functional in B.thuringiensis and E.coli, respectively. The homology of these sequences is about 70%.

The invention also relates to a sequence of nucleotides coding for the following sequence (II) of amino acids (amino acids 1-250 SEQ ID NO:2):

                                   MET  GLU  GLU  ASN  ASN  GLN  ASN GLN  CYS  ILE  PRO  TYR  ASN  CYS  LEU  SER  ASN  PRO  GLU  GLU  VAL LEU  LEU  ASP  GLY  GLU  ARG  ILE  SER  THR  GLY  ASN  SER  SER  ILE ASP  ILE  SER  LEU  SER  LEU  VAL  GLN  PHE  LEU  VAL  SER  ASN  PHE VAL  PRO  GLY  GLY  PHE  LEU  VAL  GLY  LEU  ILE  ASP  PHE  VAL  TRP GLY  ILE  VAL  GLY  PRO  SER  GLN  TRP  ASP  ALA  PHE  LEU  VAL  GLN ILE  GLU  GLN  LEU  ILE  ASN  GLU  ARG  ILE  ALA  GLU  PHE  ALA  ARG ASN  ALA  ALA  ILE  ALA  ASN  LEU  GLU  GLY  LEU  GLY  ASN  ASN  PHE ASN  ILE  TYR  VAL  GLU  ALA  PHE  LYS  GLU  TRP  GLU  GLU  ASP  PRO ASN  ASN  PRO  GLU  THR  ARG  THR  ARG  VAL  ILE  ASP  PRG  PHE  ARG ILE  LEU  ASP  GLY  LEU  LEU  GLU  ARG  ASP  ILE  PRO  SER  PHE  ARG ILE  SER  GLY  PHE  GLU  VAL  PRO  LEU  LEU  SER  VAL  TYR  ALA  GLN ALA  ALA  ASN  LEU  HIS  LEU  ALA  ILE  LEU  ARG  ASP  SER  VAL  ILE PHE  GLY  GLU  ARG  TRP  GLY  LEU  THR  THR  ILE  ASN  VAL  ASN  GLU ASN  TYR  ASN  ARG  LEU  ILE  ARG  HIS  ILE  ASP  GLU  TYR  ALA  ASP HIS  CYS  ALA  ASN  THR  TYR  ASN  ARG  GLY  LEU  ASN  ASN  LEU  PRO LYS  SER  THR  TYR  GLN  ASP  TRP  ILE  THR  TYR  ASN  ARG  LEU  ARG ARG  ASP  LEU  THR  LEU  THR  VAL  LEU  ASP  ILE  ALA  ALA  PHE  PHE PRO  ASN  TYR  ASP

A better identification of the sequence of nucleotides isolated from the above strains, deposited with the NCCM has made it possible to observe that the nucleotide situated at position 273 is guanine (G), the amino acid resulting from the GTA codon thus being valine.

Now, the reading of the nucleotide corresponding to this position 273 in the application FR.8708090 of Jun. 10, 1987 had led to reporting thymine (T) and leucine as amino acid resulting from the TTA codon.

Another sequence of nucleotides of the invention is characterized by its capacity of hybridization with a probe formed from the sequence (III) showing the following chain arrangement (SEQ ID NO:1):

  1 AAG  CTT  CAA  TAG  AAT  CTC  AAA  TCT  CGA  TGA  CTG  CTT  AGT  CTT  TTT  AAT  ACT  GTC  TAC  TTG  ACA  GGG  GTA  GGA  ACA  TAA  TCG  GTC  AAT  TTT  91 AAA  TAT  GGG  GCA  TAT  ATT  GAT  ATT  TTA  TAA  AAT  TTG  TTA  CGT  TTT  TTG  TAT  TTT  TTC  ATA  AGA  TGT  GTC  ATA  TGT  ATT  AAA  TCG  TGG  TAA 181 TGA  AAA  ACA  GTA  TCA  AAC  TAT  CAG  AAC  TTT  GGT  AGT  TTA  ATA  AAA  AAA  CGG  AGG  TAT  TTT  ATG  GAG  GAA  AAT  AAT  CAA  AAT  CAA  TGC  ATA 271 CCT  TAC  AAT  TGT  TTA  AGT  AAT  CCT  GAA  GAA  GTA  CTT  TTG  GAT  GGA  GAA  CGG  ATA  TCA  ACT  GGT  AAT  TCA  TCA  ATT  GAT  ATT  TCT  CTG  TCA 361 CTT  GTT  CAG  TTT  CTG  GTA  TCT  AAC  TTT  GTA  CCA  GGG  GGA  GGA  TTT  TTA  GTT  GGA  TTA  ATA  GAT  TTT  GTA  TGG  GGA  ATA  GTT  GGC  CCT  TCA 451 CAA  TGG  GAT  GCA  TTT  CTA  GTA  CAA  ATT  GAA  CAA  TTA  ATT  AAT  GAA  AGA  ATA  GCT  GAA  TTT  GCT  AGG  AAT  GCT  GCT  ATT  GCT  AAT  TTA  GAA 541 GGA  TTA  GGA  AAC  AAT  TTC  AAT  ATA  TAT  GTG  GAA  GCA  TTT  AAA  GAA  TGG  GAA  GAA  GAT  CCT  AAT  AAT  CCA  GCA  ACC  AGG  ACC  AGA  GTA  ATT 631 GAT  CGC  TTT  CGT  ATA  CTT  GAT  GGG  CTA  CTT  GAA  AGG  GAC  ATT  CCT  TCG  TTT  CGA  ATT  TCT  GGA  TTT  GAA  GTA  CCC  CTT  TTA  TCC  GTT  TAT 721 GCT  CAA  GCG  GCC  AAT  CTG  CAT  CTA  GCT  ATA  TTA  AGA  GAT  TCT  GTA  ATT  TTT  GGA  GAA  AGA  TGG  GGA  TTG  ACA  ACG  ATA  AAT  GTC  AAT  GAA 811 AAC  TAT  AAT  AGA  CTA  ATT  AGG  CAT  ATT  GAT  GAA  TAT  GCT  GAT  CAC  TGT  GCA  AAT  ACG  TAT  AAT  CGG  GGA  TTA  AAT  AAT  TTA  CCG  AAA  TCT 901 ACG  TAT  CAA  GAT  TGG  ATA  ACA  TAT  AAT  CGA  TTA  CGG  AGA  GAC  TTA  ACA  TTG  ACT  GTA  TTA  GAT  ATC  GCC  GCT  TTC  TTT  CCA  AAC  TAT  GAC 991 AAT  AGG  AGA  TAT  CCA  ATT  CAG  CCA  GTT  GGT  CAA  CTA  ACA  AGG  GAA  GTT  TAT  ACG  GAC  CCA  TTA  ATT  AAT  TTT  AAT  CCA  CAG  TTA  CAG  TCT 1081 GTA  GCT  CAA  TTA  CCT  ACT  TTT  AAC  GTT  ATG  GAG  AGC  AGC  GCA  ATT  AGA  AAT  CCT  CAT  TTA  TTT  GAT  ATA  TTG  AAT  AAT  CTT  ACA  ATC  TTT 1171 ACG  GAT  TGG  TTT  AGT  GTT  GGA  CGC  AAT  TTT  TAT  TGG  GGA  GGA  CAT  CGA  GTA  ATA  TCT  AGC  CTT  ATA  GGA  GGT  GGT  AAC  ATA  ACA  TAT  CCT 1261 ATA  TAT  GGA  AGA  GAG  GCG  AAC  CAG  GAG  CCT  CCA  AGA  TCC  TTT  ACT  TTT  AAT  GGA  CCG  GTA  TTT  AGG  ACT  TTA  TCA  ATT  CCT  ACT  TTA  CGA 1351 TTA  TTA  CAG  CAA  CCT  TGC  CAG  CGC  CAC  CAT  TTT  AAT  TTA  CGT  GGT  GGT  GAA  GGA  GTA  GAA  TTT  TCT  ACA  CCT  ACA  AAT  AGC  TTT  ACG  TAT 1441 CGA  GGA  AGA  GGT  ACG  GTT  GAT  TCT  TTA  ACT  GAA  TTA  CCG  CCT  GAG  GAT  AAT  AGT  GTG  CCA  CCT  CGC  GAA  GGA  TAT  AGT  CAT  CGT  TTA  TGT 1531 CAT  GCA  ACT  TTT  GTT  CAA  AGA  TCT  GGA  ACA  CCT  TTT  TTA  ACA  ACT  GGT  GTA  GTA  TTT  TCT  TGG  ACG  CAT  CGT  AGT  GCA  ACT  CTT  ACA  AAT 1621 ACA  ATT  GAT  CCA  GAG  AGA  ATT  AAT  CAA  ATA  CCT  TTA  GTG  AAA  GGA  TTT  AGA  GTT  TGG  GGG  GGC  ACC  TCT  GTC  ATT  ACA  GGA  CCA  GGA  TTT 1711 ACA  GGA  GGG  GAT  ATC  CTT  CGA  AGA  AAT  ACC  TTT  GGT  GAT  TTT  GTA  TCT  CTA  CAA  GTC  AAT  ATT  AAT  TCA  CCA  ATT  ACC  CAA  AGA  TAC  CGT 1801 TTA  AGA  TTT  CGT  TAC  GCT  TCC  AGT  AGG  GAT  GCA  CGA  GTT  ATA  GTA  TTA  ACA  GGA  GCG  GCA  TCC  ACA  GGA  GTG  GGA  GGC  CAA  GTT  AGT  GTA 1891 GAT  ATG  CCT  CTT  CAG  AAA  ACT  ATG  GAA  ATA  GGG  GAG  AAC  TTA  ACA  TCT  AGA  ACA  TTT  AGA  TAT  ACC  GAT  TTT  AGT  AAT  CCT  TTT  TCA  TTT 1981 AGA  GCT  AAT  CCA  GAT  ATA  ATT  GGG  ATA  AGT  GAA  CAA  CCT  CTA  TTT  GGT  GCA  GGT  TCT  ATT  AGT  AGC  GGT  GAA  CTT  TAT  ATA  GAT  AAA  ATT 2071 GAG  ATT  ATT  CTA  GCA  GAT  GCA  ACA  TTT  GAA  GCA  GAA  TCT  GAT  TTA  GAA  AGA  GCA  CAA  AAG  GCG  GTG  AAT  GCC  CTG  TTT  ACT  TCT  TCC  AAT 2161 CAA  ATC  GGG  TTA  AAA  ACC  GAT  GTG  ACG  GAT  TAT  CAT  ATT  GAT  CAA  GTA  TCC  AAT  TTA  GTG  GAT  TGT  TTA  TCA  GAT  GAA  TTT  TGT  CTG  GAT 2251 GAA  AAG  CGA  GAA  TTG  TCC  GAG  AAA  GTC  AAA  CAT  GCG  AAG  CGA  CTC  AGT  GAT  GAG  CGG  AAT  TTA  CTT  CAA  GAT  CCA  AAC  TTC  AGA  GGG  ATC 2341 AAT  AGA  CAA  CCA  GAC  CGT  GGC  TGG  AGA  GGA  AGT  ACA  GAT  ATT  ACC  ATC  CAA  GGA  GGA  GAT  GAC  GTA  TTC  AAA  GAG  AAT  TAC  GTC  ACA  CTA 2431 CCG  GGT  ACC  GTT  GAT  GAG  TGC  TAT  CCA  ACG  TAT  TTA  TAT  CAG  AAA  ATA  GAT  GAG  TCG  AAA  TTA  AAA  GCT  TAT  ACC  CGT  TAT  GAA  TTA  AGA 2521 GGG  TAT  ATC  GAA  GAT  AGT  CAA  GAC  TTA  GAA  ATC  TAT  TTG  ATC  GCG  TAC  AAT  GCA  AAA  CAC  GAA  ATA  GTA  AAT  GTG  CCA  GGC  ACG  GGT  TCC 2611 TTA  TGG  CCG  CTT  TCA  GCC  CAA  AGT  CCA  ATC  GGA  AAG  TGT  GGA  GAA  CCG  AAT  CGA  TGC  GCG  CCA  CAC  CTT  GAA  TGG  AAT  CCT  GAT  CTA  GAT 2701 TGT  TCC  TGC  AG

In a distinctive manner, sequences of nucleotides of the invention coding for a polypeptide toxic specifically towards larvae of Lepidoptera of the Noctuidae family, and preferably toward S.littoralis comprise or are constituted by the chain arrangement (III) previously defined.

The chain arrangement (III), comprised in the sequence of nucleotides of the invention contains 2711 nucleotides. This fragment includes in particular the potential promoter of the gene of the δ-endotoxin active on S.littoralis.

Sequences of nucleotides modified in relation to the chain arrangements (I) or (III) described above naturally enter into the framework of the present invention to the extent to which these modifications do not generate appreciable variations of the toxicity of the polypeptide coded by the modified sequence towards S.littoralis.

These modifications may, for example, consist of deletions, substitutions, recombinations.

Thus, the sequences of nucleotides (I) and (III) contain at their position 611 a variable nucleotide corresponding to adenine (A) in the sequence (I) and to cytosine (C) in the sequence (III). These nucleotides enter into the composition of the respective codons GAA and GCA which code respectively for the amino acids glutamic acid (GLU) and alanine (ALA) in the respective sequences II and IV.

Similarly, any sequence of nucleotides which can hybridize with that of the chain arrangements (I) or (III) such as obtained by reverse enzymatic transformation of the corresponding RNA or even by chemical synthesis also enter into the framework of the definitions of the invention.

The sequence of nucleotides of formula (III) starts with a ATG initiation codon situated at position 241 and which represents the start of an open reading frame of 2470 nucleotides.

The invention also relates to a sequence of nucleotides characterized in that it codes for a polypeptide containing the sequence (IV) of amino acids below (SEQ ID NO:2):

                                                                                                    MET  GLU  GLU  ASN  ASN  GLN  ASN  GLN  CYS  ILE 271 PRO  TYR  ASN  CYS  LEU  SER  ASN  PRO  GLU  GLU  VAL  LEU  LEU  ASP  GLY  GLU  ARG  ILE  SER  THR  GLY  ASN  SER  SER  ILE  ASP  ILE  SER  LEU  SER 361 LEU  VAL  GLN  PHE  LEU  VAL  SER  ASN  PHE  VAL  PRO  GLY  GLY  GLY  PHE  LEU  VAL  GLY  LEU  ILE  ASP  PHE  VAL  TRP  GLY  ILE  VAL  GLY  PRO  SER 451 GLN  TRP  ASP  ALA  PHE  LEU  VAL  GLN  ILE  GLU  GLN  LEU  ILE  ASN  GLU  ARG  ILE  ALA  GLU  PHE  ALA  ARG  ASN  ALA  ALA  ILE  ALA  ASN  LEU  GLU 541 GLY  LEU  GLY  ASN  ASN  PHE  ASN  ILE  TYR  VAL  GLU  ALA  PHE  LYS  GLU  TRP  GLU  GLU  ASP  PRO  ASN  ASN  PRO  ALA  THR  ARG  THR  ARG  VAL  ILE 631 ASP  ARG  PHE  ARG  ILE  LEU  ASP  GLY  LEU  LEU  GLU  ARG  ASP  ILE  PRO  SER  PHE  ARG  ILE  SER  GLY  PHE  GLU  VAL  PRO  LEU  LEU  SER  VAL  TYR 721 ALA  GLN  ALA  ALA  ASN  LEU  HIS  LEU  ALA  ILE  LEU  ARG  ASP  SER  VAL  ILE  PHE  GLY  GLU  ARG  TRP  GLY  LEU  THR  THR  ILE  ASN  VAL  ASN  GLU 811 ASN  TYR  ASN  ARG  LEU  ILE  ARG  HIS  ILE  ASP  GLU  TYR  ALA  ASP  HIS  CYS  ALA  ASN  THR  TYR  ASN  ARG  GLY  LEU  ASN  ASN  LEU  PRO  LYS  SER 901 THR  TYR  GLN  ASP  TRP  ILE  THR  TYR  ASN  ARG  LEU  ARG  ARG  ASP  LEU  THR  LEU  THR  VAL  LEU  ASP  ILE  ALA  ALA  PHE  PHE  PRO  ASN  TYR  ASN 991 ASN  ARG  ARG  TYR  PRO  ILE  GLN  PRO  VAL  GLY  GLN  LEU  THR  ARG  GLU  VAL  TYR  GHR  ASP  PRO  LEU  ILE  ASN  PRO  ASN  PRO  GLN  LEU  GLN  SER 1081 VAL  ALA  GLN  LEU  PRO  THR  PHE  ASN  VAL  MET  GLU  SER  SER  ALA  ILE  ARG  ASN  PRO  HIS  LEU  PHE  ASP  ILE  LEU  ASN  ASN  LEU  THR  ILE  PHE 1171 THR  ASP  TRP  PHE  SER  VAL  GLY  ARG  ASN  PHE  TYR  TRP  GLY  GLY  HIS  ARG  VAL  ILE  SER  SER  LEU  ILE  GLY  GLY  GLY  ASN  ILE  THR  SER  PRO 1261 ILE  TYR  GLY  ARG  GLU  ALA  ASN  GLN  GLU  PRO  PRO  ARG  SER  PHE  THR  PHE  ASN  GLY  PRO  VAL  PHE  ARG  THR  LEU  SER  ILE  PRO  THR  LEU  ARG 1351 LEU  LEU  GLN  GLN  PRO  CYS  GLN  ARG  HIS  HIS  PHE  ASN  LEU  ARG  GLY  GLY  GLU  GLY  VAL  GLU  PHE  SER  THR  PRO  THR  ASN  SER  PHE  THR  TYR 1441 ARG  GLY  ARG  GLY  THR  VAL  ASP  SER  LEU  THR  GLU  LEU  PRO  PRO  GLU  ASP  ASN  SER  VAL  PRO  PRO  ARG  GLU  GLY  TYR  SER  HIS  ARG  LEU  CYS 1531 HIS  ALA  THR  PHE  VAL  GLN  ARG  SER  GLY  THR  PRO  PHE  LEU  THR  THR  GLY  VAL  VAL  PHE  SER  TRP  THR  HIS  ARG  SER  ALA  THR  LEU  THR  ASN 1621 THR  ILE  ASP  PRO  GLU  ARG  ILE  ASN  GLN  ILE  PRO  LEU  VAL  LYS  GLY  PHE  ARG  VAL  TRP  GLY  GLY  THR  SER  VAL  ILE  THR  GLY  PRO  GLY  PHE 1711 THR  GLY  GLY  ASP  ILE  LEU  ARG  ARG  ASN  THR  PHE  GLY  ASP  PHE  VAL  SER  LEU  GLN  VAL  ASN  ILE  ASN  SER  PRO  ILE  THR  GLN  ARG  TYR  ARG 1801 LEU  ARG  PHE  ARG  TYR  ALA  SER  SER  ARG  ASP  ALA  ARG  VAL  ILE  VAL  LEU  THR  GLY  ALA  ALA  SER  THR  GLY  VAL  GLY  GLY  GLN  VAL  SER  VAL 1891 ASN  MET  PRO  LEU  GLN  LYS  THR  MET  GLU  ILE  GLY  GLU  ASN  LEU  THR  SER  ARG  THR  PHE  ARG  TYR  THR  ASP  PHE  SER  ASN  PRO  PHE  SER  PHE 1981 ARG  ALA  ASN  PRO  ASP  ILE  ILE  GLY  ILE  SER  GLU  GLN  PRO  LEU  PHE  GLY  ALA  GLY  SER  ILE  SER  SER  GLY  GLU  LEU  TYR  ILE  ASP  LYS  ILE 2071 GLU  ILE  ILE  LEU  ALA  ASP  ALA  THR  PHE  GLU  ALA  GLU  SER  ASP  LEU  GLU  ARG  ALA  GLN  LYS  ALA  VAL  ASN  ALA  LEU  PHE  THR  SER  SER  ASN 2161 GLN  ILE  GLY  LEU  LYS  THR  ASP  VAL  THR  ASP  TYR  HIS  ILE  ASP  GLN  VAL  SER  ASN  LEU  VAL  ASP  CYS  LEU  SER  ASP  GLU  PHE  CYS  LEU  ASP 2251 GLU  LYS  ARG  GLU  LEU  SER  GLU  LYS  VAL  LYS  HIS  ALA  LYS  ARG  LEU  SER  ASP  GLU  ARG  ASN  LEU  LEU  GLN  ASP  PRO  ASN  PHE  ARG  GLY  ILE 2341 ASN  ARG  GLN  PRO  ASP  ARG  GLY  TRP  ARG  GLY  SER  THR  ASP  ILE  THR  ILE  GLN  GLY  GLY  ASP  ASP  VAL  PHE  LYS  GLU  ASN  TYR  VAL  THR  LEU 2431 PRO  GLY  THR  VAL  ASP  GLU  CYS  TYR  PRO  THR  TYR  LEU  TYR  GLN  LYS  ILE  ASP  GLU  SER  LYS  LEU  LYS  ALA  TYR  THR  ARG  TYR  GLU  LEU  ARG 2521 GLY  TYR  ILE  GLU  ASP  SER  GLN  ASP  LEU  GLU  ILE  TYR  LEU  ILE  ALA  TYR  ASN  ALA  LYS  HIS  GLU  ILE  VAL  ASN  VAL  PRO  GLY  THR  GLY  SER 2611 LEU  TRP  PRO  LEU  SER  ALA  GLN  SER  PRO  ILE  GLY  LYS  CYS  GLY  GLU  PRO  ASN  ARG  CYS  ALA  PRO  HIS  LEU  GLU  TRP  ASN  PRO  ASP  LEU  ASP 2701 CYS  SER  CYS

The invention also relates to recombinant expression and cloning vectors comprising more particularly at least one sequence of nucleotides such as that defined above, in particular at least a part of the sequence of about 3 kb.

A specific recombinant vector is, for example, a plasmid containing the HindIII-PstI fragment of the sequence of nucleotides of the invention, inserted in a vector pUC9. A first preferred vector is the plasmid pHT71, the construction of which is reported in the assemblies below, which comprises a HindIII-PstI DNA fragment according to the invention constituted uniquely of DNA derived from the strain aizawai 7-29.

Another recombinant vector is constituted by the plasmid pHT 671, the construction of which is given in FIG. 4. This plasmid contains a chimeric HindIII-PstI fragment, obtained by fusing a HindIII-HindII fragment of 1.1 kb derived from the strain entomocidus 6-01 with a HincII-PstI fragment of 1.9 kb derived from the strain aizawai 7-29.

The modified bacterial strains which contain one of the nucleotide sequences defined above or also a recombinant expression vector and cloning previously defined, and preferably the plasmid pHT671 or the plasmid pHT71, also enter into the framework of the invention.

The invention also relates to a polypeptide toxic towards larvae of Lepidoptera and in a preferential manner towards S.littoralis, which attack cotton leaves or other crops such as those listed above, characterized in that it is capable of forming an immunological complex with antibodies directed against polypeptides with larvicidal activity towards S.littoralis.

The invention relates more particularly to the NH₂-terminal part of this polypeptide which contains the larvicidal activity.

The extremity of the active NH₂-terminal part corresponds to the sequence (II) of amino acids given above.

A preferred polypeptide of the invention is that which corresponds to this sequence (II) and corresponds to the sequence (IV) of amino acids given in the preceding pages. This polypeptide corresponding to the sequence (IV) contains 823 amino acids. Its calculated molecular mass is 92906 Da.

This sequence of δ-endotoxin was compared with amino acid sequences of δ-endotoxins derived from other strains of B.thuringiensis active on the Lepidoptera and the genes of which have been isolated and sequenced previously: the δ-endotoxins in question are those of the strains kurstaki HD1 (19), kurstaki HD73 (20), berliner 1715 (21) and (22) Sotto (23) and aizawai IPL7 (24).

The results of these comparisons indicate that all are different in the second quarter of the molecule (amino acids 281 to 620) whereas the NH₂-terminal part (amino acids 1 to 280) and the COOH-terminal domain (amino acids 621 to 1175) of the protein are highly conserved and differ only by several amino acids. On the other hand, the δ-endotoxin corresponding to the sequence (IV) above shows considerable differences from the other δ-endotoxins both in the NH₂-terminal part (amino acids 1 to 280) and in the second quarter of the molecule (amino acids 281 to 620). The results of these comparisons indicate again that the NH₂-terminal half of the molecule (amino acids 1 to 620) which corresponds to the toxic fraction of the protein only show 46% homology with the other δ-endotoxins. The most important differences are located in the second half of the toxic part of the molecule (amino acids 281 to 620) with only 36% of identical amino acids, the NH₂-terminal part (amino acids 1 to 280) itself showing 58% of amino acids identical with the other δ-endotoxins. Such considerable differences have never been observed up to now in the NH₂ terminal part of the toxic fraction of the molecule among the δ-endotoxins active on the Lepidoptera.

In order to obtain a sequence of nucleotides entering into the framework of the invention, coding for at least the active part of a polypeptide showing a specific toxicity towards larvae of Lepidoptera of the Noctuidae family, and preferably towards S.littoralis, recourse is had, in conformity with the invention, to the following steps, namely:

the carrying out of a molecular hybridization between, on the one hand, a nucleotide sequence of a strain of B.thuringiensis active against S.littoralis and, on the other, at least two nucleotide sequences, used as probes, derived from the 5′ part of a restriction fragment of a gene for δ-endotoxin of B.thuringiensis, this part coding for the NH₂-terminal part of the polypeptide active on the larvae of Lepidoptera, and from the 3′ part of this fragment coding for the COOH part of the polypeptide,

the isolation of the hybrid fragment,

its cloning in a vector, followed by its purification.

In an advantageous manner, the hybridization probes utilized are obtained from a gene for the δ-endotoxin derived from the strain aizawai 7-29 coding for a protein of 130 kDa, active against P.brassicae and inactive towards S.littoralis, this gene having been cloned in the recombinant plasmid pHTA2.

In an embodiment of the preceding procedure, the fragment recombined with the vector in the cloning step is elaborated from a HindIII-PstI restriction fragment derived from a single strain of B.thuringiensis, preferably aizawai 7-29. In particular, this fragment is carried preferentially by the recombinant plasmid pHTA6 such as isolated with the aid of a probe constituted by a PvuII fragment of 2 kb of the plasmid pBT15-88 corresponding to the internal part of a gene for the chromosomal crystal of the strain berliner 1715, starting from transforming clones containing nucleotide sequences derived from B.thuringiensis strains active against larvae of Lepidoptera, inter-alia of S.littoralis.

In another embodiment of the invention, the fragment recombined with the vector in the cloning step is elaborated from several sequences of nucleotides derived from recombinant vectors containing sequences of nucleotides from at least two different strains of B.thuringiensis, possessing the same restriction maps and themselves containing all or part of the sequences of nucleotides capable of coding for a polypeptide active, in a preferential manner, against S.littoralis.

In this case, the recombined fragment used in the cloning step is a fragment of about 3 kb, advantageously elaborated from a HindIII-HincII restriction fragment of about 1.1 kb derived from the entomocidus 6-01 strain and a HincII-PstI fragment of about 1.9 kb from the aizawai 7-29 strain. It corresponds to a truncated gene for δ-endotoxin.

The HindIII-HincII and HincII-PstI restriction fragments are carried more especially by the respective recombinant plasmids pHTE6 and pHTA6 such as isolated with the aid of the probe constituted by the PvuII fragment mentioned above.

The study of the toxicity towards the larvae of Lepidoptera of the bacterial strains modified with the aid of the sequences of nucleotides defined above, has made it possible to demonstrate their high toxic activity, in particular with regard to the caterpillars of S.littoralis.

This activity was estimated from the point of view of the specificity index corresponding to the ratio

LC50 S.littoralis/LC50 P.brassicae

in which “LC50” represents the lethal concentration killing 50% of the larvae in 72 hours.

The utilization of such an index makes it possible to evaluate the activity of the bacterial strains studied without having to consider the level of expression of the polypeptides.

The results obtained, which are reported in the examples which follow, and the values of LD50 which are deduced from them, have shown that the bacterial strains modified according to the invention show a more specific toxic activity towards S.littoralis than the native crystal proteins of the strains aizawai 7-29 or berliner 1715.

Therefore, the invention relates to the use of these modified strains, of recombinant vectors containing the nucleotide sequences defined above, in particular the plasmid pHT671 and the plasmid pHT71, and these sequences themselves for the elaboration of larvicidal compositions preferentially toxic towards S.littoralis.

The larvicidal compositions of the invention are thus characterized in that they contain an efficaceous quantity of polypeptides such as defined above or expressed by the nucleotide sequences mentioned above.

In order to produce these polypeptides the truncated genes for δ-endotoxin corresponding to the nucleotide sequences of the invention are advantageously implemented.

These genes can be used to produce in excess the toxic polypeptide in microorganisms permitting the expression of the above recombinant vectors. Suitable strains of microorganisms include E.coli or also B.subtilis.

These truncated genes may be reintroduced into the strains of B.thuringiensis or into related species such as B.cereus, according to the standard techniques, for example, by transformation, conjugation or transduction. These techniques make it possible to produce the toxic polypeptide in large quantity without first having to modify the natural region of the promoter for the δ-endotoxin genes of B.thuringiensis.

This transformation may be carried out by using methods derived from the transformation of the protoplasts of B.subtilis according to (11) or of the vegetative cells of B.thuringiensis as described in (12).

The introduction of recombinant plasmids by a system of the conjugation type may be carried out by using B.thuringiensis as host strain and B.subtilis or Streptococcus faecalis as strains of the donor type by operating according to (13) and (14).

As a variant, the sequences of nucleotides are introduced into microorganisms living in the environment or in association with the plants and capable of expressing recombinant vectors containing these sequences. The introduction may be carried out in microorganisms such as Pseudomonas by working according to the procedure described in (17), by the intermediary of plasmid vectors containing the transposon Tn5 and the gene for the toxin, or Azospirillum or Rhizobium by means of the intermediary of suicide vectors derived from the plasmid RP4 and of mobilizing plasmids functional in Gram negative bacteria (for example, pRK2013) according to the procedures described in (18).

The truncated genes are alone in the strains of Bacilli or, as a variant, are associated with different δ-endotoxin genes which makes it possible to obtain crystals synthesized by these strains specifically toxic towards given species of Noctuidae, or toxic both towards the Noctuidae and insects sensitive to other δ-endotoxins. These recombinations, carried out in vitro or in vivo with the nucleotide sequences of the invention and other δ-endotoxin genes showing different toxic specificities, lead to the construction of new genes coding for novel hybrid toxic proteins exhibiting a large spectrum of activity towards insects. These new genes and these novel proteins also enter into the framework of the invention.

In these applications, the nucleotide sequences of the invention may be transferred and expressed in plants sensitive to S.littoralis in order to diminish the devastation caused by these insects.

Among the plants to be protected, mention should be made of: cotton, clover, the tomatoe and alfalfa.

The transfer of the truncated gene into cotton plants may be carried out by transformation involving strains such as Agrobacterium as described in (15).

In addition, the invention relates to the plant cells, the plants and the seeds containing the nucleotide sequences defined above.

The plant cells according to the invention are cells, the genome of which after transformation by a non-essentially biological procedure possesses in a stable manner a sequence of nucleotides capable of expressing a polypeptide toxic towards S.littoralis, such as that defined above. The invention also relates to the plant cells derived from their division.

The plants according to the invention are plants transformed by a non-essentially biological procedure, having in particular as predator S.littoralis, the genome of which possesses in a stable manner a sequence of nucleotides such as that defined above, capable of expressing a polypeptide toxic towards S.littoralis. The plants in question are also plants derived from their reproduction, their multiplication or hybrid crosses.

In accordance with another feature, the invention relates to plants having in particular as predator S.littoralis, possessing in addition to their initial phenotypic and genotypic characters the property of expressing a polypeptide toxic preferentially towards S.littoralis, this property resulting from the insertion in their genome by means of genetic manipulation of a sequence of nucleotides capable of expressing the said polypeptide.

In addition, the invention relates to seeds capable of giving rise to a plant such as that defined above or derived from such a plant, characterized in that they have integrated into their genome by genetic manipulation a nucleotide sequence described above.

BRIEF DESCRIPTION OF THE DRAWINGS

Other characteristics and advantages of the invention will become apparent in the course of the description and in referring to the examples.

FIG. 1 presents the restriction map of the plasmids pHTA6 and pHTE6.

FIG. 2 depicts the restriction map of a gene for a crystal protein of the aizawai 7-29 strain cloned in the plasmid pHTA2 and defines the DNA fragments which are used as probes.

FIG. 3 shows the fragment of 6.6 kb cloned in pHTA2 and the results of a hybridization carried out between this fragment and the probes described in FIG. 2.

FIG. 4 depicts the restriction map of the plasmid pHT671.

FIG. 5 shows the photographs of the immunodiffusion tests. In FIG. 5A an antiserum against all of the δ-endotoxins of aizawai 7-29, containing rabbit antibodies directed against the solubilized crystal protein, was used in the central well. In FIG. 5B, an antiserum containing rabbit polyclonal antibodies against the crystal proteins of Berliner 1715 was used. In FIGS. 5A and 5B, solubilized, purified crystal of aizawai 7-29 was placed in well No. 1 to serve as a positive control and wells No. 2, 3, 4, 5, and 6 contained E. coli clones containing the plasmids pHT671, pHTA4, pHTA2, pHT71 and pUC18, respectively.

EXAMPLE 1 Construction of a DNA Sequence of About 3 kb Containing a Hybrid Gene of an Insecticidal Toxin

This construction comprises:

1/ the preparation of gene banks of B.thuringiensis

2/ the selection and characterization of transforming clones containing the genes of a crystal protein and nucleotide sequences responsible for the larvicidal activity,

3/ in vitro recombination of these sequences in a cloning vector with construction of the plasmid pHT671.

These different steps are carried out as follows:

1/ Preparation of Gene Banks of B.thuringiensis

The total DNA of the aizawai 7-29 and entomocidus 6-01 strains of Bacillus thuringiensis is purified by using the method reported in (1) and 50 μg of each purified DNA are completely digested with the restriction enzyme PstI.

The DNA digested by PstI is analysed by horizontal electro-phoresis on a 0.8% agarose gel and DNA fragments of a size of 5 to 8 kb are recovered from the agarose gels by electroelution in a manner described in (2).

The purified DNA fragments of 5-8 kb of the aizawai 7-29 strain are ligated to the DNA of the cloning vector pUC18 digested by PstI according to (3).

The purified DNA fragments of 5-8 kb of the entomocidus 6-01 chain are ligated to the DNA of the cloning vector pUC9 digested by PtI. The cells of E.coli JM83 are transformed with the ligation mixture as described in (4).

The transforming clones of E.coli are selected on LB medium containing 100 μg/ml of ampicillin.

2/ Isolation and Characterization of the Transforming Clones Containing the Genes for a Crystal Protein

A/ Screening of the transformed E.coli cells with the aid of an internal fragment of a gene of the crystal protein labelled with ³²P, used as probe:

Transforming clones containing recombinant plasmids carrying the gene for the crystal are detected by colony hybridization according to the method described in (5), by using as probe a PvuII fragment of 2 kb of the pBT 15-88 plasmid corresponding to an internal part of the gene for the crystal protein located on the chromosome of the berliner 1715 strain.

B/ Characterization of the recombinant plasmids present in the clones which react with the above probe.

Two recombinant plasmids, pHTA6 and pHTE6, isolated respectively from gene banks constructed from the strains aizawai 7-29 and entomocidus 6-01, show a homology with this probe. In each case, a DNA fragment of about 6.6 kb was cloned.

The restriction map of the two plasmids is given in FIG. 1. The comparison of the restriction sites shows that the two DNA fragments cloned appear to be identical.

In order to delimit the sequences corresponding to the gene for the δ-endotoxin, different DNA fragments labelled with ³²P, derived from a gene of the crystal previously characterized, and cloned in the recombinant plasmid pHTA2, are utilized as probes. This latter gene for the crystal also derived from the aizawai 7-29 strain codes for a protein of 130 kd active against P.brassicae but not against S.littoralis. This type of gene possesses the same restriction map as the gene for the δ-endotoxin derived from the berliner 1715 strain. In FIG. 2 is shown the restriction map of this gene for the crystal protein of the aizawai 7-29 strain cloned in the plasmid pHTA2. The thick lines shown above the map correspond to the fragments used as hybridization probes.

The plasmids pHTA6 and pHTE6 are hydrolysed by different restriction endonucleases, analysed by horizontal electrophoresis on a 0.8% agarose gel and hybridized with the different probes.

The transfer of the DNA to nitrocellulose filters is carried out according to the method of SOUTHERN described in (6). The hybridization is conducted at 42° C. for 24 hours in a solution containing: 5×SSC, 30% formamide and a 1×Denhardt mixture described in (7) in the presence of a DNA probe labelled with ³²P. The filters are then washed at 42° C. for 20 minutes, by using successively the following solutions: 5 SSC in 50% formamide, 5 SSC, 2 SSC, 1 SSC and 0.5 SSC before being dried at room temperature.

The results of these hybridization experiments are summarized in FIG. 3. It appears that each extremity of the cloned DNA fragments of 6.6 kb shows a homology with the probes. The PstI-KpnI fragment of 1.5 kb reacting with the probe No. 3 corresponds to the 3′ end of a gene of the crystal protein present in both the aizawai 7-29 and entomocidus 6-01 strains. As pointed out in FIG. 3, the probes No. 1 and No. 2 corresponding to the 5′ end of the gene for the δ-endotoxin of pHTA2 hybridize with the HindIII-HincII fragment of 1.1 kb contained in the plasmid pHTA6. The probe No. 3 which covers the 3′ end of the gene of the δ-endotoxin of pHTA2 hybridizes with the HindIII-PstI fragment of 0.4 kb contained in the plasmid pHTA6. It should be noted that a weak hybridization signal is obtained with the probe No. 2 whereas the two other probes give easily detectable signals.

From these results, the inventors have established that the HindIII-PstI DNA fragment of 3 kb corresponds to a large part of a gene for the δ-endotoxin which commences close to the central HindIII site. It seems clear in the light of results of the hybridization experiments that the gene for the δ-endotoxin shows substantial differences from those characterized in the prior art. On the basis of these results it was decided to clone the HindIII-PstI fragment of 3 kb in the vector pUC9.

3/ Construction of the Plasmid pHT 671 Containing a Hybrid Gene of the Reconstituted Insecticidal Toxin

The HindIII-HincII DNA fragment of 1.1 kb derived from the plasmid pHTE6 and the HincII-PstI DNA fragment of 1.9 kb derived from the plasmid pHTA6 are purified on agarose gels.

Equal amounts of the two purified DNA fragments and the DNA of pUC9 digested with HindIII and PstI are mixed and ligated. The ligation mixture is used to transform competent cells of E.coli JM83, then the transformed E.coli cells are selected on LB medium containing ampicillin. One of the interesting recombinant clones examined contains a plasmid designated by pHT671, the restriction map of which was determined and is shown in FIG. 4. This plasmid (pHT671) contains a DNA fragment of 3 kb inserted in the vector pUC9. This DNA sequence has the same restriction map as the HindIII-PstI fragments of 3 kb contained in the plasmids pHTA6 and pHTE6, but corresponds to a reconstituted DNA molecule constructed by in vitro recombination from DNA sequences derived from the aizawai 7-29 strains on the one hand and entomocidus 6-01 on the other.

EXAMPLE II Study of the Nucleotide Sequence of the Promoter Region and of the Region Coding for the NH₂-Terminal Part of the δ-Endotoxin Active Against the Noctuidae

The HindIII-HincII fragment of pHT671 is sequenced in conformity with the method described in (8) by using a M13 system. In order to obtain partially overlapping cloned DNA fragments which will be used in the sequencing of the DNA, recourse is had to the method of subcloning by deletion in M13, developed by DALE et al (9).

The sequence of 940 nucleotides of the HindIII-HincII fragment which has a length of about 1 kilobase corresponds to the chain arrangement I above.

The analysis of this sequence shows that the largest open reading frame starts at position 241 and that a potential site of binding to the ribosomes, GGAGG, is found six base pairs upstream from this ATG codon (position 230 to 235). The region localized between the nucleotides 137 and 177 (position -103 to -63 upstream from the ATG codon) is strongly homologous with the region present upstream from the gene for the crystal of the strain kurstaki HD1 Dipel (BTX) sequenced by WONG et al (1983) and described in (16) and the authors of which have shown that it contains three promoters BtI, BtII, and Ec, functional in B.thuringiensis and E.coli, respectively. The comparison between the amino acid sequences deduced from the first 750 nucleotides of the genes of BTK and pHT671, show that these polypeptides exhibit significant differences at the level of the N-terminal half of the active part derived from the protoxin (only 66% strict homology). It is important to note that it is the first time that a gene for the δ-endotoxin isolated from a strain active against the Lepidoptera codes for a polypeptide which shows substantial differences in this region. In fact, this N-terminal domain appears to be strongly conserved (more than 97% of strict homology) among all of the genes for the crystal active on Lepidoptera which have been sequenced hitherto. Moreover, the inventors have shown that the degree of variability is of the same order if the nucleotide sequences of pHT671 and other genes of the Lepidoptera type are considered.

EXAMPLE III Construction of a DNA Sequence of About 2.7 kb Containing a Gene for a Larvicidal Toxin

In order to achieve this construction the DNA of the aizawai 7-29 strain of B.thuringiensis was used up to the step for the production of the plasmid pHTA6 as described in Example I.

The HindIII-PstI fragment of about 2.7 kb obtained from the plasmid pHTA6 was then subcloned in the vector pUC9, previously hydrolysed by the restriction enzymes HindIII-PstI in order to give the plasmid pHT71.

EXAMPLE IV Study of the Sequence of Nucleotides Constituting the Plasmid pHT71 Coding for a Polypeptide Toxic Towards the Larvae of Lepidoptera of the Family of the Noctuidae

The HindIII-PstI fragment of 2.7 kb of pHTA6, which was subcloned in pHT71, was sequenced by means of the technique of Sanger et al. (8) using the phage M13mp19 and the subcloning system by deletions developed by Dale et al (9). This system makes it possible to obtain M13 phages containing a series of partially overlapping DNA fragments which can be utilized for sequencing the DNA.

The sequence of nucleotides of this 2.7 kb fragment which corresponds to the chain arrangement (III) given above, was determined on the 2 DNA strands, with the. exception of the last 212 nucleotides (position 2500 to 2711) which were sequenced only on a single strand.

The nucleotide sequence of this HindIII-PstI fragment has a length of 2711 nucleotides. This fragment contains the potential promoter as well as the largest part of the gene for the δ-endotoxin active on S.littoralis.

EXAMPLE V Study of the Specific Toxicity of the Recombinant Clones of E. Coli JM83 (pHT671) and JM83 (pHT71) Against S.littoralis

The toxicity of the recombinant clones of E.coli JM83 containing pHT671 and of E.coli JM83 containing pHT71 was determined by biological tests on caterpillars of the P.brassicae and S.littoralis species as described by LECADET and MARTOURET in (10). The results were compared with the specific toxicity of the native crystal proteins purified from the strains berliner 1715 and aizawai 7-29, entomocidus 6-01 B.cereus 569 (containing the plasmid pBT45, pAMβ1) against the two species of insects. The specific toxicity of the recombinant clone and of the strains of B.thuringiensis is expressed in terms of “specificity index” previously defined.

The results obtained are reported in table 1 below.

In this table, for E.coli strains, the concentration 1 corresponds to a 14 hours bacterial culture concentrated 20 times, disintegrated by ultrasound; for the B.thuringiensis strains the concentration is expressed in μg of crystal protein per μl of preparation. The toxic activity of the preparations was tested by the forced ingestion with 5 μl of preparation on caterpillars at the fifth stage of development, or by a technique of free ingestion utilizing larvae at the second stage of development.

TABLE 1 Comparative toxicity of a recombinant clone and two strains of B. thuringiensis towards S. littoralis and P. brassicae. P. S. littoralis brassicae Specificity index LC50 LC50 LC50 LC50 S. littoralis Strains 2nd larval 5th larval 5th larval LC50 and plasmids stage stage stage P. brassicae JM83 (pUC18) >1 >1 >1 — JM83 (pHT671) 0.04 0.13 0.72 0.2 JM83 (pHTA2) >1 >1 0.03 >30 JM83 (pHTA4) >1 >1 >1 — JM83 (pHT71) ND 0.5 >1 <0.5 berliner 1715 ND 0.11 0.007 15.7 native crystals aizawai 7.29 ND 0.02 0.04 0.5 native crystals entomocidus 601 ND 0.028 0.012 2.3 native crystals B. cereus 569 ND 0.38 0.054 7 (pBT45, pAMβ 1)

Examination of the LC50 values summarized in this table 1 shows that the protein extracts of the recombinant clones JM83 (pHT671) and JM83 (pHT71) are preferentially toxic against S.littoralis. Secondly, a comparison of the values of the specificity index shows that the larvicidal activity of the recombinant clones is more specific by a factor of 2.5 times towards S.littoralis than the native crystal proteins of the aizawai strain. Moreover, the recombinant clones of JM83 (pHT671) and DI83 (pHT71) are very active against another insect of the family of the Noctuidae, Mamestra brassicae (in the case of the clone JM83 (pHT671) for example, the LC50 value is 0.02, utilizing larvae at the second stage of development).

These two results show that the gene for the larvicidal toxin constructed and cloned in the plasmids pHT671 and pHT71 codes for a protein specifically active against S.littoralis.

Other preparations obtained from recombinant clones containing plasmids carrying genes coding for other types of δ-endotoxins (pHTA2 and pHTA4) are not active on S.littoralis: it may be seen that the plasmid pHTA2 codes for a δ-endotoxin specifically active on P.brassicae whereas the plasmid pHTA4 codes for a δ-endotoxin, the insect target for which has not yet been identified. It can also be seen that the crystalline inclusions produced by a strain of Bacillus cereus which has received the plasmid pBT45, one of the plasmids of the aizawai 7-29 strain which also carries a δ-endotoxin gene (the gene of plasmid origin of the aizawai 7-29 strain), are also specifically active on P.brassicae.

Similar results are obtained by using, in the place of crude bacterial extracts, soluble protein extracts prepared from different recombinant clones of E.coli.

On the basis of the LC50 values reported in the table above and a mean individual weight of 41 mg per L5 larva (fifth larval stage) of S.littoralis, the value of the LD50 was estimated at 2.4 pg/gram of larva for the native crystals of the aizawai 7-29 strain.

On these same bases and on the basis of equivalence factors making it possible to pass from the total bacterial mass to the quantity of specific proteins (about 2% of the total proteins in E.coli JM83 (pHT671), the LD50 corresponding to the toxin produced by the expression in E.coli JM83 of the gene according to the invention cloned in the plasmid pHT671, was determined and estimated at a value close to 5.5 to 6 μg/gram of larva.

On these same bases and after determination of the LC50 of soluble protein extracts prepared from ground cultures of E.coli JM83 (pHT671), the value of the LD50 corresponding to the toxin present in these extracts was estimated at 4.15 μg/gram of larva.

In the two cases and particularly in the case of the ground preparations of E.coli, the calculated values of LD50 are approximate and higher than that of the native crystals, because it is not a question of a purified toxin. However, these data indicate without ambiguity that the gene expressed by pHT671 specifies a δ-endotoxin exhibiting the specificity towards S.littoralis. In fact, the same type of estimation made with extract of E.coli JM83 (pHTA2) carrying a δ-endotoxin gene of different specificity leads to values 30 to 50 times higher than the LD50 of the soluble extracts towards S.littoralis (135 to 350 μg/gram of larva).

The foregoing data will easily make it possible for the person skilled in the art to develop active larvicidal compositions with the proteins of the invention.

Other toxicity experiments were carried out utilizing larvae of M.brassicae, S.fruqiperda and S.littoralis at the second larval stage. The results obtained, expressed in terms of LC50 as defined for table 1, are given in table 2.

TABLE 2 ACTIVITY OF THE RECOMBINANT CLONES AGAINST THE LARVAE OF INSECTS OF THE FAMILY OF THE NOCTUIDAE: M. BRASSICAE, S. FRUGIPERDA, and S. LITTORALIS. INSECT LARVAE AND STAGE M. BRASSICAE S. FRUGIPERDA S. LITTORALIS STRAINS AND LC50 LC50 LC50 PLASMIDS 2nd STAGE 2nd STAGE 2nd STAGE JM 83 (pUC18) NT NT NT JM 83 (pHTA2) >1 0.51 0.9 JM 83 (pHT671) 0.02 0.5  0.03 JM 83 (pHT71) ND ND 0.03 JM 83 (pHTA4) >1 0.54 >1

It emerges from the examination of table 2 that the crude bacterial extracts of the recombinant clone JM83 (pHT671) are toxic towards M.brassicae and S.littoralis (the values of LC50 are 0.02 and 0.03, respectively) and weakly toxic towards S.fruqiperda (LC50 of 0.5).

The extracts of the recombinant clone E.coli JM83 (pHTA2) are weakly active towards S.fruqiperda and S.littoralis and not at all toxic towards M.brassicae. The extracts of the recombinant clone JM83 (pHTA4) are not toxic towards M.brassicae and S.littoralis and are weakly toxic toward S.fruqiperda.

These results confirm the high specific toxicity of the proteins obtained from pHT71 and pHT671 towards S.littoralis and show that this class of crystal protein is also very active towards M.brassicae.

EXAMPLE VI Study of the Specificity of the Polypeptides Expressed by the Clones Formed by Introduction of the Plasmids pHT671 and pHT71 into E.coli

This study was carried out owing to immuno-diffusion tests. The results are reported in FIG. 5 (which includes FIGS. 5A and 5B).

The implementation of the immuno-diffusion experiment was done in conformity with the following protocol:

Soluble extracts of proteins of E.coli clones containing the plasmids pHT671, pHTA4, pHTA2 or pHT71, pUC18 were placed in the wells Nos. 2, 3, 4, 5, 6, respectively. A sample of a solubilized purified crystal of aizawai 7-29 was placed in the well No. 1 in order to serve as positive control.

In the test recorded in FIG. 5A an antiserum against all of the δ-endotoxins of aizawai 7-29, containing rabbit antibodies directed against the solubilized crystal proteins, was used and placed in the central well.

An immunoprecipitation line was observed in all of the cases except in the case of the extract of E.coli containing only the plasmid vector (well No. 6).

It was observed that the immuno-precipitation lines derived from the wells No. 4 and No. 5 cross, which shows that the products encoded by the plasmids pHTA2 and pHT71, respectively, display different antigenic determinants.

In the test recorded in FIG. 5B, the anti-serum used contained rabbit polyclonal antibodies against the crystal proteins of berliner 1715.

An immunoprecipitation line was observed with the extracts of E.coli JM83 (pHTA4) (well No. 3) JM83 (pHTA2) (well No. 4). On the other hand, the E.coli clones JM83 (pHT71) (well No. 5), JM83 (pHT671) (well No. 2) or JM83 (pUC9) (well No. 6) did not give immunoprecipitation.

It may be deduced from that that the genes for the crystal isolated in pHTA4 and pHTA2 express polypeptides having antigenic determinants in common with the proteins of the crystal of berliner 1715, a strain which is not specifically active towards S.littoralis.

On the other hand, the crude extracts of E.coli containing the plasmids pHT671 and pHT71 contain polypeptides having antigenic determinants in common with the crystal proteins of the aizawai 7-29 strain, which are not related immunogenically with the crystal proteins of the berliner 1715 strain.

These results confirm those given previously with respect to the specificity of the genes isolated in the plasmids pHT71 and pHT671.

Antigen-antibody precipitation assays have made it possible to determine the level of expression of the δ-endotoxin genes in different recombinant clones.

The results obtained have shown that the crystal protein represents between 7 and 10% of the total cellular proteins of E.coli JM83 (pHTA2), between 2 and 3% in E.coli JM83 (pHT671) and between 0.5 and 1% in E.coli JM83 (pHTA4) and E.coli JM83 (pHT71).

The literature references cited in the examples are the following:

(1) KLIER, A. F., LECADET, M-M. and DEDONDER, R., 1973, Sequential modifications of RNA polyzerase during sporogenesis in Bacillus thuringiensis, Eur. J. Biochem., 36: 317-327.

(2) MANIATIS, T., FRITSCH, E. F. , SAMBROOK, J., 1982, Molecular cloning: A laboratory manual. Cold Spring Harbor Laboratory Press, New-York

(3) VIEIRA, J. and MESSING, J., 1982, The pUC plasmids, and M13mp7 derived system for insertion mutagenesis and sequencing with synthetic universal primers, Gene, 19: 259-268.

(4) LEDERBERG, E. M. and COHEN, S. N. , 1974, Transformation of Salmonella typhimurium by plasmid deoxyribonucleic acid, J. Bacteriol., 119: 1072-1074.

(5) GRUNSTEIN, M. and HOGNESS, D. S. , 1975, Colony hybridization, a method for the isolation of cloned DNAs that contain a specific gene, Proc. Natl. Acad. Sci. U.S.A., 72: 3961-3965:

(6) SOUTHERN, E. M. , 1975, Detection of specific sequence among DNA fragments separated by gel electrophoresis, J. Molec. Biol., 98, 503-517.

(7) DENHARDT, D. T. 1976, A membrane filter taking for the detection of complementary DNA. Biochem. Biophys. Res. Comm., 23: 641-646.

(8) SANGER, F., NICKLENS, S. and COULSON, A. R. , 1977, DNA sequencing with chain terminating inhibitors. Proc. Natl. Acad. Sci. U. S. A., 74: 5463-5467.

(9) DALE et al. (1985) A rapid single-stranded cloning strategy for producing a sequential series of overlapping clones for use in DNA, Plasmid 1985, 13: 31-40

(10) LECADET.M. M. et MARTOURET D. 1987, Hcst specificity of the Bacillus thuringiensis δ-endotoxin toward Lepidopteran species: Spodoptera littoralis Bdv and Pieris brassicae L, J. of Invert. Pathol., 49 (n^(o)1): 37-48.

(11) CHANG et al., 1979, High frequency transformation of Bacillus subtilis protoplasts by plasmid DNA-Mol Gen Genet 168:111 115

(12) HEIFRSON et al., 1987, Transformation of vegetative cells of Bacillus thuringiensis by plasmid DNA, Journal of Bacteriology, March 1987, p.1147-1152,

(13) KLIER et al., 1983, Mating between Bacillus subtilis and Bacillus thuringiensis and transfer of cloned crystal genes, Mol Gen Genet (1983) 191:257 262

(14) LERECLUS et al., 1983, Isolation of a DNA, sequence related to several plasmids from Bacillus thuringiensis after a mating involving the Streptococcus faecalis plasmid pAMβ1, Mol Gen Genet (1983) 191:307-313

(15) UMBECK et al., 1987, Genetically transformed cotton (Gossypium hirsutum L.) plants—Biotechnology vol.5 March 1987.

(16) WONG et al., 1983, transcriptional and translational start sites for the Bacillus thuringiensis crystal protein gene. J. of Biol. Chem., 258: 1960-1967.

(17) OBUKOWICZ M.et al (1986). Tn⁵ mediated integration of the δ-endotoxin gene from B. thuringiensis into the chromosome of root colonizing Pseudomonas. J. Bacteriol., 168, 982-989.

(18) SIMON, R. et al, (1983). A broad host range mobilization system for in vivo genetic engineering: transposon mutagenesis in Gram-negative bacteria. Biotechnology, 1, pp. 784-791.

(19) Schnepf et al, (1985) The amino acid sequence of a crystal protein from Bacillus thuringiensis deduced from the DNA base sequence. J BIOL Chem 260: 6264-6372.

(20) Adang et al, (1985) characterized full-length and truncated plasmid clones of the crystal protein of Bacillus thuringiensis subsp. kurstaki HD-73 and their toxicity to Manduca sexta. Gene 46: 289-300.

(21) Wabiko et al, (1986) Bacillus thuringiensis entomocidal protoxin gene sequence and gene product analysis. DNA 5: 305-314.

(22) Hofte et al, (1986) Structural and functional analysis of a cloned δ-endotoxin gene of Bacillus thuringiensis berliner 1715. Eur J Biochem 161: 273-280.

(23) Shibano et al, (1986) Complete structure of an insecticidal crystal protein gene from Bacillus thuringiensis. In: Bacillus molecular genetics and biotechnology applications. J. Ganesan, A. T., Hoch, J. A.(eds). Academic Press 307-320.

(24) Oeda et al, (1987) Nucleotide sequence of the insecticidal protein gene of Bacillus thuringiensis strain aizawai IPL7 and its high-level expression in Escherichia coli. Gene 53: 113-119.

2 2711 base pairs nucleic acid single linear DNA (genomic) 1 AAGCTTCAAT AGAATCTCAA ATCTCGATGA CTGCTTAGTC TTTTTAATAC TGTCTACTTG 60 ACAGGGGTAG GAACATAATC GGTCAATTTT AAATATGGGG CATATATTGA TATTTTATA 120 AATTTGTTAC GTTTTTTGTA TTTTTTCATA AGATGTGTCA TATGTATTAA ATCGTGGTA 180 TGAAAAACAG TATCAAACTA TCAGAACTTT GGTAGTTTAA TAAAAAAACG GAGGTATTT 240 ATGGAGGAAA ATAATCAAAA TCAATGCATA CCTTACAATT GTTTAAGTAA TCCTGAAGA 300 GTACTTTTGG ATGGAGAACG GATATCAACT GGTAATTACT CAATTGATAT TTCTCTGTC 360 CTTGTTCAGT TTCTGGTATC TAACTTTGTA CCAGGGGGAG GATTTTTAGT TGGATTAAT 420 GATTTTGTAT GGGGAATAGT TGGCCCTTCT CAATGGGATG CATTTCTAGT ACAAATTGA 480 CAATTAATTA ATGAAAGAAT AGCTGAATTT GCTAGGAATG CTGCTATTGC TAATTTAGA 540 GGATTAGGAA ACAATTTCAA TATATATGTG GAAGCATTTA AAGAATGGGA AGAAGATCC 600 AATAATCCAG CAACCAGGAC CAGAGTAATT GATCGCTTTC GTATACTTGA TGGGCTACT 660 GAAAGGGACA TTCCTTCGTT TCGAATTTCT GGATTTGAAG TACCCCTTTT ATCCGTTTA 720 GCTCAAGCGG CCAATCTGCA TCTAGCTATA TTAAGAGATT CTGTAATTTT TGGAGAAAG 780 TTGGGATTGA CAACGATAAA TGTCAATGAA AACTATAATA GACTAATTAG GCATATTGA 840 GAATATGCTG ATCACTGTGC AAATACGTAT AATCGGGGAT TAAATAATTT ACCGAAATC 900 ACGTATCAAG ATTGGATAAC ATATAATCGA TTACGGAGAG ACTTAACATT GACTGTATT 960 GATATCGCCG CTTTCTTTCC AAACTATGAC AATAGGAGAT ATCCAATTCA GCCAGTTG 1020 CAACTAACAA GGGAAGTTTA TACGGACCCA TTAATTAATT TTAATCCACA GTTACAGT 1080 GTAGCTCAAT TACCTACTTT TAACGTTATG GAGAGCAGCG CAATTAGAAA TCCTCATT 1140 TTTGATATAT TGAATAATCT TACAATCTTT ACGGATTGGT TTAGTGTTGG ACGCAATT 1200 TATTGGGGAG GACATCGAGT AATATCTAGC CTTATAGGAG GTGGTAACAT AACATCTC 1260 ATATATGGAA GAGAGGCGAA CCAGGAGCCT CCAAGATCCT TTACTTTTAA TGGACCGG 1320 TTTAGGACTT TATCAATTCC TACTTTACGA TTATTACAGC AACCTTGCCA GCGCCACC 1380 TTTAATTTAC GTGGTGGTGA AGGAGTAGAA TTTTCTACAC CTACAAATAG CTTTACGT 1440 GCAGGAAGAG GTACGGTTGA TTCTTTAACT GAATTACCGC CTGAGGATAA TAGTGTGC 1500 CCTCGCGAAG GATATAGTCA TCGTTTATGT CATGCAACTT TTGTTCAAAG ATCTGGAA 1560 CCTTTTTTAA CAACTGGTGT AGTATTTTCT TGGACGCATC GTAGTGCAAC TCTTACAA 1620 ACAATTGATC CAGAGAGAAT TAATCAAATA CCTTTAGTGA AAGGATTTAG AGTTTGGG 1680 GGCACCTCTG TCATTACAGG ACCAGGATTT ACAGGAGGGG ATATCCTTCG AAGAAATA 1740 TTTGGTGATT TTGTATCTCT ACAAGTCAAT ATTAATTCAC CAATTACCCA AAGATACC 1800 TTAAGATTTC GTTACGCTTC CAGTAGGGAT GCAGCAGTTA TAGTATTAAC AGGAGCGG 1860 TCCACAGGAG TGGGAGGCCA AGTTAGTGTA GATATGCCTC TTCAGAAAAC TATGGAAA 1920 GGGGAGAACT TAACATCTAG AACATTTAGA TATACCGATT TTAGTAATCC TTTTTCAT 1980 AGAGCTAATC CAGATATAAT TGGGATAAGT GAACAACCTC TATTTGGTGC AGGTTCTA 2040 AGTAGCGTTG AACTTTATAT AGATAAAATT GAAATTATTC TAGCAGATGC AACATTTG 2100 GCAGAATCTG ATTTAGAAAG AGCACAAAAG GCGGTGAATG CCCTGTTTAC TTCTTCCA 2160 CAAATCGGGT TAAAAACCGA TGTGACGGAT TATCATATTG ATCAAGTATC CAATTTAG 2220 GATTGTTTAT CAGATGAATT TTGTCTGGAT GAAAAGCGAG AATTGTCCGA GAAAGTCA 2280 CATGCGAAGC GACTCAGTGA TGAGCGGAAT TTACTTCAAG ATCCAAACTT CAGAGGGA 2340 AATAGACAAC CAGACCGTGG CTGGAGAGGA AGTACAGATA TTACCATCCA AGGAGGAG 2400 GACGTATTCA AAGAGAATTA CGTCACACTA CCGGGTACCG TTGATGAGTG CTATCCAA 2460 TATTTATATC AGAAAATAGA TGAGTCGAAA TTAAAAGCTT ATACCCGTTA TGAATTAA 2520 GGGTATATCG AAGATAGTCA AGACTTAGAA ATCTATTTGA TCGCGTACAA TGCAAAAC 2580 GAAATAGTAA ATGTGCCAGG CACGGGTTCC TTATGGCCGC TTTCAGCCCA AAGTCCAA 2640 GGAAAGTGTG GAGAACCGAA TCGATGCGCG CCACACCTTG AATGGAATCC TGATCTAG 2700 TGTTCCTGCA G 2711 823 amino acids amino acid unknown unknown peptide 2 Met Glu Glu Asn Asn Gln Asn Gln Cys Ile Pro Tyr Asn Cys Leu Se 1 5 10 15 Asn Pro Glu Glu Val Leu Leu Asp Gly Glu Arg Ile Ser Thr Gly As 20 25 30 Ser Ser Ile Asp Ile Ser Leu Ser Leu Val Gln Phe Leu Val Ser As 35 40 45 Phe Val Pro Gly Gly Gly Phe Leu Val Gly Leu Ile Asp Phe Val Tr 50 55 60 Gly Ile Val Gly Pro Ser Gln Trp Asp Ala Phe Leu Val Gln Ile Gl 65 70 75 80 Gln Leu Ile Asn Glu Arg Ile Ala Glu Phe Ala Arg Asn Ala Ala Il 85 90 95 Ala Asn Leu Glu Gly Leu Gly Asn Asn Phe Asn Ile Tyr Val Glu Al 100 105 110 Phe Lys Glu Trp Glu Glu Asp Pro Asn Asn Pro Ala Thr Arg Thr Ar 115 120 125 Val Ile Asp Arg Phe Arg Ile Leu Asp Gly Leu Leu Glu Arg Asp Il 130 135 140 Pro Ser Phe Arg Ile Ser Gly Phe Glu Val Pro Leu Leu Ser Val Ty 145 150 155 160 Ala Gln Ala Ala Asn Leu His Leu Ala Ile Leu Arg Asp Ser Val Il 165 170 175 Phe Gly Glu Arg Trp Gly Leu Thr Thr Ile Asn Val Asn Glu Asn Ty 180 185 190 Asn Arg Leu Ile Arg His Ile Asp Glu Tyr Ala Asp His Cys Ala As 195 200 205 Thr Tyr Asn Arg Gly Leu Asn Asn Leu Pro Lys Ser Thr Tyr Gln As 210 215 220 Trp Ile Thr Tyr Asn Arg Leu Arg Arg Asp Leu Thr Leu Thr Val Le 225 230 235 240 Asp Ile Ala Ala Phe Phe Pro Asn Tyr Asp Asn Arg Arg Tyr Pro Il 245 250 255 Gln Pro Val Gly Gln Leu Thr Arg Glu Val Tyr Thr Asp Pro Leu Il 260 265 270 Asn Phe Asn Pro Gln Leu Gln Ser Val Ala Gln Leu Pro Thr Phe As 275 280 285 Val Met Glu Ser Ser Ala Ile Arg Asn Pro His Leu Phe Asp Ile Le 290 295 300 Asn Asn Leu Thr Ile Phe Thr Asp Trp Phe Ser Val Gly Arg Asn Ph 305 310 315 320 Tyr Trp Gly Gly His Arg Val Ile Ser Ser Leu Ile Gly Gly Gly As 325 330 335 Ile Thr Ser Pro Ile Tyr Gly Arg Glu Ala Asn Gln Glu Pro Pro Ar 340 345 350 Ser Phe Thr Phe Asn Gly Pro Val Phe Arg Thr Leu Ser Ile Pro Th 355 360 365 Leu Arg Leu Leu Gln Gln Pro Cys Gln Arg His His Phe Asn Leu Ar 370 375 380 Gly Gly Glu Gly Val Glu Phe Ser Thr Pro Thr Asn Ser Phe Thr Ty 385 390 395 400 Arg Gly Arg Gly Thr Val Asp Ser Leu Thr Glu Leu Pro Pro Glu As 405 410 415 Asn Ser Val Pro Pro Arg Glu Gly Tyr Ser His Arg Leu Cys His Al 420 425 430 Thr Phe Val Gln Arg Ser Gly Thr Pro Phe Leu Thr Thr Gly Val Va 435 440 445 Phe Ser Trp Thr His Arg Ser Ala Thr Leu Thr Asn Thr Ile Asp Pr 450 455 460 Glu Arg Ile Asn Gln Ile Pro Leu Val Lys Gly Phe Arg Val Trp Gl 465 470 475 480 Gly Thr Ser Val Ile Thr Gly Pro Gly Phe Thr Gly Gly Asp Ile Le 485 490 495 Arg Arg Asn Thr Phe Gly Asp Phe Val Ser Leu Gln Val Asn Ile As 500 505 510 Ser Pro Ile Thr Gln Arg Tyr Arg Leu Arg Phe Arg Tyr Ala Ser Se 515 520 525 Arg Asp Ala Arg Val Ile Val Leu Thr Gly Ala Ala Ser Thr Gly Va 530 535 540 Gly Gly Gln Val Ser Val Asn Met Pro Leu Gln Lys Thr Met Glu Il 545 550 555 560 Gly Glu Asn Leu Thr Ser Arg Thr Phe Arg Tyr Thr Asp Phe Ser As 565 570 575 Pro Phe Ser Phe Arg Ala Asn Pro Asp Ile Ile Gly Ile Ser Glu Gl 580 585 590 Pro Leu Phe Gly Ala Gly Ser Ile Ser Ser Gly Glu Leu Tyr Ile As 595 600 605 Lys Ile Glu Ile Ile Leu Ala Asp Ala Thr Phe Glu Ala Glu Ser As 610 615 620 Leu Glu Arg Ala Gln Lys Ala Val Asn Ala Leu Phe Thr Ser Ser As 625 630 635 640 Gln Ile Gly Leu Lys Thr Asp Val Thr Asp Tyr His Ile Asp Gln Va 645 650 655 Ser Asn Leu Val Asp Cys Leu Ser Asp Glu Phe Cys Leu Asp Glu Ly 660 665 670 Arg Glu Leu Ser Glu Lys Val Lys His Ala Lys Arg Leu Ser Asp Gl 675 680 685 Arg Asn Leu Leu Gln Asp Pro Asn Phe Arg Gly Ile Asn Arg Gln Pr 690 695 700 Asp Arg Gly Trp Arg Gly Ser Thr Asp Ile Thr Ile Gln Gly Gly As 705 710 715 720 Asp Val Phe Lys Glu Asn Tyr Val Thr Leu Pro Gly Thr Val Asp Gl 725 730 735 Cys Tyr Pro Thr Tyr Leu Tyr Gln Lys Ile Asp Glu Ser Lys Leu Ly 740 745 750 Ala Tyr Thr Arg Tyr Glu Leu Arg Gly Tyr Ile Glu Asp Ser Gln As 755 760 765 Leu Glu Ile Tyr Leu Ile Ala Tyr Asn Ala Lys His Glu Ile Val As 770 775 780 Val Pro Gly Thr Gly Ser Leu Trp Pro Leu Ser Ala Gln Ser Pro Il 785 790 795 800 Gly Lys Cys Gly Glu Pro Asn Arg Cys Ala Pro His Leu Glu Trp As 805 810 815 Pro Asp Leu Asp Cys Ser Cys 820 

What is claimed is:
 1. A method for obtaining a nucleotide sequence that codes for the active part of a polypeptide toxic for larvae of S. littoralis, wherein the method comprises: (A) hybridizing at least one nucleotide probe to DNA from a strain of B. thuringiensis active against S. littoralis, wherein the nucleotide probe from the 5′ end of a restriction fragment of a gene for δ endotoxin of B. thuringiensis strain aizawa 7-29, and wherein the nucleotide probe comprises the HincII-PstI fragment of the δ endotoxin of B. thuringiensis strain aizawa 7-29 and further comprises the HindIII-HincII restriction fragment of B. thuringiensis strain entomocidus 6-01; (B) isolating the DNA from the strain of B. thuringiensis active against S. littoralis that hybridized to the probe; (C) cloning the isolated DNA into a vector; and (D) purifying the vector to thereby obtain the nucleotide sequence that codes for the active part of a polypeptide toxic for larvae of S. littoralis. 